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  • C12N2500/70—Undefined extracts
  • C12N2500/74—Undefined extracts from fungi, e.g. yeasts

Definitions

• the present invention relates generally to cell culture medium formulations. Specifically, the present invention provides cell culture medium formulations which comprise one or more plant peptides for facilitating the in vitro cultivation of animal cells.
• the present invention also relates to media formulations which comprise one or more plant lipids and/or fatty acids for cultivation of animal cells in vitro.
• the formulations of the invention may also comprise one or more plant peptides and one or more plant lipids or fatty acids. In accordance with the invention, such plant-derived peptides, lipids and/or fatty acids may be used as substitutes for one or a number of animal-derived culture media components.
• the invention also provides methods for cultivating animal cells using these plant nutrient-based culture media.
• the media of the present invention are particularly suited for virus production in animal cells.
• Cell culture media provide the nutrients necessary to maintain and grow cells in a controlled, artificial and in vitro environment. Characteristics and compositions of the cell culture media vary depending on the particular cellular requirements. Important parameters include osmolarity, pH, and nutrient formulations.
• Media formulations have been used to cultivate a number of cell types including animal, plant and bacterial cells.
• Cells cultivated in culture media catabolize available nutrients and produce useful biological substances such as monoclonal antibodies, hormones, growth factors and the like. Such products have therapeutic applications and, with the advent of recombinant DNA technology, cells can be engineered to produce large quantities of these products.
• Cultured cells are also routinely used for the isolation, identification and growth of viruses.
• the ability to cultivate cells in vitro is not only important for the study of cell physiology, but is also necessary for the production of useful substances which may not otherwise be obtained by cost-effective means.
• Typical components of cell culture media include amino acids, organic and inorganic salts, vitamins, trace metals, sugars, lipids and nucleic acids, the types and amounts of which may vary depending upon the particular requirements of a given cell or tissue type.
• cell culture media formulations are supplemented with a range of additives, including undefined components such as fetal bovine serum (FBS) (10-20% v/v) or extracts from animal embryos, organs or glands (0.5-10% v/v). While FBS is the most commonly applied supplement in animal cell culture media, other serum sources are also routinely used, including newborn calf, horse and human. These types of chemically undefined supplements serve several useful functions in cell culture media ( Lambert, K.J. et al., In: Animal Cell Biotechnology, Vol. 1, Spier, R.E. et al., Eds., Academic Press New York, pp. 85-122 (1985 )).
• FBS fetal bovine serum
• these supplements provide carriers or chelators for labile or water-insoluble nutrients; bind and neutralize toxic moieties; provide hormones and growth factors, protease inhibitors and essential, often unidentified or undefined low molecular weight nutrients; and protect cells from physical stress and damage.
• serum and/or animal extracts are commonly used as relatively low-cost supplements to provide an optimal culture medium for the cultivation of animal cells.
• Cell surface chemistry which is a critical portion of the in vitro microenvironment for many cell types, can be adversely modified via adsorption or incorporation of serum or extract proteins.
• the use of undefined components such as serum or animal extracts also prevents the true definition and elucidation of the nutritional and hormonal requirements of the cultured cells, thus eliminating the ability to study, in a controlled way, the effect of specific growth factors or nutrients on cell growth and differentiation in culture.
• undefined supplements prevent the researcher from studying aberrant growth and differentiation and the disease-related changes in cultured cells.
• serum and animal extract supplementation of culture media can also complicate and increase the costs of the purification of the desired substances from the culture media due to nonspecific co-purification of serum or extract proteins.
• serum-free media which often are specifically formulated to support the culture of a single cell type, incorporate defined quantities of purified growth factors, lipoproteins and other proteins usually provided by the serum or extract supplement.
• SFM serum-free media
• SFM generally provide several distinct advantages to the user. For example, the use of SFM facilitates the investigation of the effects of a specific growth factor or other medium component on cellular physiology, which may be masked when the cells are cultivated in serum- or extract-containing media. In addition, SFM typically contain much lower quantities of protein (indeed, SFM are often termed "low protein media") than those containing serum or extracts, rendering purification of biological substances produced by cells cultured in SFM far simpler and more cost-effective.
• SFM small cell culture
• Such media (often called “basal media”), however, are usually seriously deficient in the nutritional content required by most animal cells. Accordingly, most SFM incorporate into the basal media additional components to make the media more nutritionally complex, but to maintain the serum-free and low protein content of the media.
• additional components include serum albumin from bovine (BSA) or human (HSA), animal-derived lipids such as human Excyte, sterols, etc., and certain growth factors or hormones derived from natural (animal) or recombinant sources.
• supplements derived from the same species as the cells to be cultured may be used.
• culture of human cells may be facilitated using HSA as a supplement, while media for the culture of bovine cells would instead use BSA.
• This approach runs the risks of introducing contaminants and adventitious pathogens into the culture medium (such as HIV or Hepatitis B virus from HSA preparations, or Bovine Spongiform Encephalopathy virus from BSA preparations), which can obviously negatively impact the use of such media in the preparation of animal and human therapeutics.
• the biotechnology industry and government agencies are increasingly regulating, discouraging and even forbidding the use of cell culture media containing animal-derived products which may contain such pathogens.
• animal cell culture media that are completely free of animal proteins.
• some culture media have incorporated extracts of yeast cells into the basal medium (see, for example, U.K. Patent Application No. GB 901673 ; Keay, L., Biotechnol. Bioengin. 17:745-764 (1975 )) to provide sources of nitrogen and other essential nutrients.
• hydrolysates of wheat gluten have been used, with or without addition of yeast extract, to promote in vitro growth of animal cells (Japanese Patent Application No. JP 2-49579 ).
• wheat peptides are known to be toxic or to induce toxic effects in vitro and in vivo, particularly in the cells and tissues of the gastrointestinal systems of some mammals, including humans ( Strober, W., et al., Ann. Int. Med. 83:242-256 (1975 ); Auricchio, S., et al., Pediatr. Res. 22(6):703-707 (1987 )).
• a serum-free, low-protein culture medium suitable for cultivation of animal cells, which is completely devoid of animal or human proteins.
• Such a medium formulation will facilitate studies of the effects of growth factors and other stimuli on cellular physiology, will allow easier and more cost-effective purification of biological substances produced by cultured animal cells in the biotechnology industry, and most importantly will eliminate the risk of the introduction of adventitious animal and human pathogens.
• the current invention provides such an animal cell culture medium formulation.
• the present invention provides culture media formulations that support the culture of animal cells comprising plant peptides, preferably as a primary protein source.
• the invention provides a cell culture medium, capable of supporting the cultivation of an animal cell in vitro, comprising at least one plant peptide which is not derived from wheat and which is most preferably derived from rice.
• the media formulations of the invention comprise at least one plant lipid and/or fatty acid.
• the media formulations of the invention may comprise at least one plant peptide and at least one plant lipid and/or fatty acid.
• the invention also provides such media formulations which further comprise an enzymatic digest or extract of yeast cells.
• the invention also provides a cell culture medium, capable of supporting the cultivation of an animal cell in vitro, comprising an extract of yeast cells wherein the medium does not further comprise a wheat-derived plant peptide.
• the media of the present invention may be 1X formulations, or may be concentrated as 10X-100X, most preferably as 10X, 20X, 25X, 50X or 100X formulations.
• the basal medium of the present invention comprises a number of ingredients, including amino acids, vitamins, organic and inorganic salts, sugars, each ingredient being present in an amount which supports the cultivation of an animal cell in vitro.
• the medium of the invention may be used to culture a variety of animal cells, including insect cells (such as from Spodoptera or Trichoplusa species), avian cells and mammalian cells (including primary cells, established cell lines, CHO cells, COS cells, VERO cells, BHK cells and human cells).
• insect cells such as from Spodoptera or Trichoplusa species
• avian cells including primary cells, established cell lines, CHO cells, COS cells, VERO cells, BHK cells and human cells.
• the present invention also provides methods of culturing animal and human cells using the culture medium formulations disclosed herein, comprising the steps of (a) contacting an animal cell with the cell culture medium of the present invention; and (b) cultivating the animal cell under conditions suitable to support its cultivation in vitro.
• the present invention also relates to methods for replacing or substituting animal-derived produces with plant peptides, plant lipids/fatty acids (or combinations thereof), and/or enzymatic digests or extracts of yeast cells.
• Such plant-derived products may be substituted for any number of animal-derived products, including but not limited to blood-derived products (e.g., serum, albumin, antibodies, fibrinogen, factor VIII, etc.), tissue or organ extracts and/or hydrolysates (e.g., bovine pituitary extract (BPE), bovine brain extract, chick embryo extract and bovine embryo extract), and animal-derived lipids and fatty acids, peptones, Excyte, sterols (e.g ., cholesterol) and lipoproteins (e.g ., high-density and low-density lipoproteins (HDLs and LDLs, respectively)).
• blood-derived products e.g., serum, albumin, antibodies, fibrinogen, factor VIII, etc.
• the invention further provides compositions comprising the culture media of the present invention and an animal cell, including any of the animal cells described above.
• ingredients refers to any compound, whether of chemical or biological origin, that can be used in cell culture media to maintain or promote the growth of proliferation of cells.
• component e.g., fetal calf serum
• ingredient e.g., calf serum, calf serum, calf serum, calf serum, calf serum, calf serum, calf serum, calf serum, calf serum, calf serum, calf serum, calfate, calfate, calfate, arate, glycerol, glycerin, glycerin, glycerin, glycerin, glycerin, glycerin, calfate, calfate, calfate, calfate, calfate, calfate, calfate, calfate, calfate, calfate, calfate, calfate, calfate, calfate, calfate, calfate,
• cytokine refers to a compound that induces a physiological response in a cell, such as growth, differentiation, senescence, apoptosis, cytotoxicity or antibody secretion. Included in this definition of "cytokine” are growth factors, interleukins, colony-stimulating factors, interferons and lymphokines.
• cell culture or “culture” is meant the maintenance of cells in an artificial, in vitro environment. It is to be understood, however, that the term “cell culture” is a generic term and may be used to encompass the cultivation not only of individual cells, but also of tissues, organs, organ systems or whole organisms, for which the terms “tissue culture,” “organ culture,” “organ system culture” or “organotypic culture” may occasionally be used interchangeably with the term “cell culture.”
• cultivation is meant the maintenance of cells in vitro under conditions favoring growth, differentiation or continued viability, in an active or quiescent state, of the cells.
• cultivation may be used interchangeably with “cell culture” or any of its synonyms described above.
• culture vessel is meant a glass, plastic, or metal container that can provide an aseptic environment for culturing cells.
• cell culture medium refers to a nutritive solution for cultivating cells and may be used interchangeably.
• extract is meant a composition comprising a concentrated preparation of the components of a substance, typically formed by treatment of the substance either mechanically (e.g., by pressure treatment) or chemically (e.g., by distillation, precipitation, enzymatic action or high salt treatment).
• enzyme digest a composition comprising a specialized type of extract, namely one prepared by treating the substance to be extracted (e.g., plant components or yeast cells) with at least one enzyme capable of breaking down the components of the substance into simpler forms (e.g., into a preparation comprising mono- or disaccharides and/or mono-, di- or tripeptides).
• substance to be extracted e.g., plant components or yeast cells
• enzyme capable of breaking down the components of the substance into simpler forms e.g., into a preparation comprising mono- or disaccharides and/or mono-, di- or tripeptides.
• hydrolysate may be used interchangeably with the term “enzymatic digest.”
• contacting refers to the placing of cells to be cultivated in vitro into a culture vessel with the medium in which the cells are to be cultivated.
• the term “contacting” encompasses mixing cells with medium, pipetting medium onto cells in a culture vessel, and submerging cells in culture medium.
• combining refers to the mixing or admixing of ingredients in a cell culture medium formulation.
• a cell culture medium is composed of a number of ingredients and these ingredients vary from one culture medium to another.
• a "1X formulation” is meant to refer to any aqueous solution that contains some or all ingredients found in a cell culture medium at working concentrations.
• the “1X formulation” can refer to, for example, the cell culture medium or to any subgroup of ingredients for that medium.
• the concentration of an ingredient in a 1X solution is about the same as the concentration of that ingredient found in a cell culture formulation used for maintaining or cultivating cells in vitro.
• a cell culture medium used for the in vitro cultivation of cells is a 1X formulation by definition. When a number of ingredients are present, each ingredient in a 1X formulation has a concentration about equal to the concentration of those ingredients in a cell culture medium.
• RPMI-1640 culture medium contains, among other ingredients, 0.2 g/L L-arginine, 0.05 g/L L-asparagine, and 0.02 g/L L-aspartic acid.
• a "1X formulation" of these amino acids contains about the same concentrations of these ingredients in solution.
• each ingredient in solution has the same or about the same concentration as that found in the cell culture medium being described.
• concentrations of ingredients in a 1X formulation of cell culture medium are well known to those of ordinary skill in the art. See Methods For Preparation of Media, Supplements and Substrate For Serum-Free Animal Cell Culture Allen R. Liss, N.Y. (1984 ), which is incorporated by reference herein in its entirety.
• the osmolarity and/or pH may differ in a 1X formulation compared to the culture medium, particularly when fewer ingredients are contained in the 1X formulation.
• a "10X formulation” is meant to refer to a solution wherein each ingredient in that solution is about 10 times more concentrated than the same ingredient in the cell culture medium.
• a 10X formulation of RPMI-1640 culture medium may contain, among other ingredients, 2.0 g/L L-arginine, 0.5 g/L L-asparagine, and 0.2 g/L L-aspartic acid (compare 1X formulation, above).
• a "10X formulation” may contain a number of additional ingredients at a concentration about 10 times that found in the 1X culture medium.
• 20X formulation designate solutions that contain ingredients at about 20-, 25-, 50- or 100- fold concentrations, respectively, as compared to a 1X cell culture medium.
• the osmolarity and pH of the media formulation and concentrated solution may vary.
• the cell culture media of the present invention are aqueous-based, comprising a number of ingredients in a solution of deionized, distilled water to form "basal media.” Any basal medium can be used in accordance with the present invention.
• Ingredients which the basal media of the present invention may include are amino acids, vitamins, organic and/or inorganic salts, trace elements, buffering salts and sugars.
• the basal media of the invention comprise one or more amino acids, one or more vitamins, one or more inorganic salts, adenine sulfate, ATP, one or more trace elements, deoxyribose, ethanolamine, D-glucose, glutathione, N-[2-hydroxyethyl]piperazine-N'-[2-ethanesulfonic acid] (HEPES) or one or more other zwitterion buffers, hypoxanthine, linoleic acid, lipoic acid, insulin, phenol red, phosphoethanolamine, putrescine, sodium pyruvate, thymidine, uracil and xanthine.
• HEPES N-[2-hydroxyethyl]piperazine-N'-[2-ethanesulfonic acid]
• HEPES N-[2-hydroxyethyl]piperazine-N'-[2-ethanesulfonic acid]
• HEPES N-[2-hydroxyethy
• Amino acid ingredients which may be included in the media of the present invention include L-alanine, L-arginine, L-asparagine, L-aspartic acid, L-cystine, L-cysteine, L-glutamic acid, L-glutamine, glycine, L-histidine, L-isoleucine, L-leucine, L-lysine, L-methionine, L-phenylalanine, L-proline, L-serine, L-threonine, L-tryptophan, L-tyrosine and L-valine. These amino acids may be obtained commercially, for example from Sigma (Saint Louis, Missouri).
• Vitamin ingredients which may be included in the media of the present invention include ascorbic acid magnesium salt, biotin, choline chloride, D-Ca ++ -pantothenate, folic acid, i -inositol, menadione, niacinamide, nicotinic acid, paraaminobenzoic acid (PABA), pyridoxal, pyridoxine, riboflavin, thiamine ⁇ HCl, vitamin A acetate, vitamin B 12 and vitamin D 2 . These vitamins may be obtained commercially, for example from Sigma (Saint Louis, Missouri).
• Inorganic salt ingredients which may be used in the media of the present invention include CaCl 2 , KCl, MgCl 2 , MgSO 4 , NaCl, NaHCO 3 , Na 2 HPO 4 , NaH 2 PO 4 ⁇ H 2 O and ferric citrate chelate or ferrous sulfate chelate. These inorganic salts may be obtained commercially, for example from Sigma (Saint Louis, Missouri).
• Trace elements which may be used in the media of the present invention include ions of barium, bromium, cobalt, iodine, manganese, chromium, copper, nickel, selenium, vanadium, titanium, germanium, molybdenum, silicon, iron, fluorine, silver, rubidium, tin, zirconium, cadmium, zinc and aluminum.
• ions may be provided, for example, in trace element salts such as Ba(C 2 H 3 O 2 ) 2 , KBr, CoCl 2 ⁇ 6H 2 O, KI, MnCl 2 ⁇ 4H 2 O, Cr(SO 4 ) 3 ⁇ 15H 2 O, CuSO 4 ⁇ 5H 2 O, NiSO 4 ⁇ 6H 2 O, H 2 SeO 3 , NaVO 3 , TiCl 4 , GeO 2 , (NH 4 ) 6 Mo 7 O 24 ⁇ 4H 2 O, Na 2 SiO 3 ⁇ 9H 2 O, FeSO 4 ⁇ 7H 2 O, NaF, AgNO 3 , RbCl, SnCl 2 , ZrOCl 2 ⁇ 8H 2 O, CdSO 4 ⁇ 8H 2 O, ZnSO 4 ⁇ 7H 2 O, Fe(NO 3 ) 3 ⁇ 9H 2 O, AlCl 3 ⁇ 6H 2 O.
• trace element salts such as Ba(C 2 H 3 O 2 ) 2
• Cytokines which may be used in the media of the present invention include growth factors such as epidermal growth factor (EGF), acidic fibroblast growth factor (aFGF), basic fibroblast growth factor (bFGF), hepatocyte growth factor (HGF), insulin-like growth factor 1 (IGF-1), insulin-like growth factor 2 (IGF-2), keratinocyte growth factor (KGF), nerve growth factor (NGF), platelet-derived growth factor (PDGF), transforming growth factor beta (TGF- ⁇ ), vascular endothelial cell growth factor (VEGF), transferrin, various interleukins (such as IL-1 through IL-18), various colony-stimulating factors (such as granulocyte/macrophage colony-stimulating factor (GM-CSF)), various interferons (such as IFN- ⁇ ) and other cytokines having effects upon hematopoietic stem cells such as stem cell factor (SCF) and erythropoietin (Epo).
• EGF epidermal
• cytokines may be obtained commercially, for example from Life Technologies, Inc. (Rockville, Maryland) or R&D Systems (Minneapolis, Minnesota), and may be either natural or recombinant. Most preferably, for culture of a wide variety of mammalian cells, the basal media will contain EGF at a concentration of about 0.1-100 nanograms/milliliter, preferably about 1-10 nanograms/milliliter, and most preferably about 5-10 nanograms per milliliter. Other cytokines, if used, may be added at concentrations that are determined empirically or as guided by the established cytokine art.
• Additional ingredients that may be included in the present media are insulin (especially as insulin ⁇ Zn ++ ) and transferrin. These additional ingredients, available commercially (e.g., from Sigma, St. Louis, Missouri), may be formulated into the present media at the concentration ranges and preferred concentrations shown in Table 1. Ferric citrate chelate or ferrous sulfate can be used in the present media as a substitute for transferrin. Additionally, recombinant insulin may be substituted for animal- or human-derived insulin. Table 1. Animal cell culture basal medium component concentrations.
• Component Component Ranges (mg/L) A Preferred Embodiment (mg/L) Most Preferred Embodiment (mg/L) Amino Acids about: about: about: L-Alanine 1-250 9 8.90 L-Arginine•HCl 10-500 400 390.0 L-Asparagine•H 2 O 5-150 41 41.01 L-Aspartic Acid 5-125 13 13.30 L-Cystine•2HCl 0.1-250 115 114.67 L-Cysteine•HCl•H 2 O 2-250 24 24.39 L-Glutamic Acid 5-250 11 10.73 Glycine 1-200 8 7.50 L-Histidine•HCl•H 2 O 5-250 68 68.29 L-Isoleucine 5-500 171 171.34 L-Leucine 25-350 180 180.44 L-Lysine•HCl 25-500 226 225.62 L-Methionine 5-200 51 50.62 L-Phenylalanine 5-250 97 96.79 L-
• basal medium When admixed together in solution, form a "basal medium.”
• Other basal media can be equivalently used in accordance with the invention.
• at least one peptide, extract, enzymatic digest or hydrolysate of plant protein, and/or at least one plant-derived lipid and/or fatty acid is added to a basal medium to formulate the complete culture media of the present invention.
• Plants suitable as sources of proteins, peptides, lipids and/or fatty acids in formulating the culture media of the present invention include, but are not limited to, rice ( Oryza sativa ), soy (Glycine max), potato (Solanum tuberosum) and corn ( Zea mays). Particularly preferred as a source of plant protein is rice.
• rice Oryza sativa
• soy Glycine max
• potato Solanum tuberosum
• corn Zea mays
• Particularly preferred as a source of plant protein is rice.
• the use of wheat as a source of plant-derived proteins is specifically excluded from the present invention, as extracts and peptide preparations from wheat have been shown to contain inhibitors of protein synthesis in animal cell systems ( Coleman, W.H., and Roberts, W.K., Biochim. Biophys.
• Plant peptides for use in formulating the culture media of the present invention may be prepared by digesting plant extracts with enzymes such as trypsin or chymotrypsin, by methods that are routine in the art.
• plant peptides in the form of enzymatic digests or hydrolysates may be obtained commercially, for example from Quest International (Norwich, New York). Plant peptides are added to the basal medium at a concentration of about 10-1000 mg/liter, preferably about 50-500 mg/liter, and most preferably about 100-200 mg/liter.
• At least one plant lipid and/or fatty acid may be added to prepare the media formulations of the invention.
• Plant lipids/fatty acids suitable for use in the present culture media may be obtained from any of the above-described plant sources and others that will be familiar to one of ordinary skill, using methods of lipid/fatty acid isolation (for example, chromatography, particularly HPLC) that are well-known in the art.
• plant lipids/fatty acids and complexes of lipids and/or fatty acids may be obtained commercially, for example from Matreya, Inc. (Pleasant Gap, Pennsylvania).
• Particularly preferred lipids/fatty acids for use in the present culture media include, but are not limited to, palmitate, stearate, oleate, linoleate, linolenate, arachidate, myristate, behenate, erucate, lignocerate, caprylate, caprate, laurate and palmitoleate.
• These lipids/fatty acids may be added individually or as mixtures comprising two or more of the above-described lipids/fatty acids, preferably in specific proportions as described in more detail below in Example 7.
• plant lipids/fatty acids are added to a basal medium at concentrations of about 0.00001 to about 10,000 ⁇ g/ml, more preferably about 0.0001 to about 1000 ⁇ g/ml, and most preferably about 0.001 to about 100 ⁇ g/ml.
• the basal medium including plant-derived peptides and/or lipids/fatty acids formulate complete culture media according to the present invention.
• These complete media are suitable for use in the culture of a variety of animal cells, as described in more detail below. It may be preferable, however, to further enrich the nutritional content of the complete media to support faster growth and enhanced production of biologicals by the cultured cells, and to provide a more suitable environment for the culture of fastidious animal cells. To accomplish such enrichment, one or more additional nutrients derived from non-animal sources may be added to the above-described basal or complete media.
• the additional nutrients added to the basal medium or complete medium may comprise extracts of yeast cells (hereinafter “yeast extract” or “YE”), and most preferably are ultrafiltered YE (hereinafter “yeast extract ultrafiltrate” or “YEU”).
• yeast extract extracts of yeast cells
• YEU ultrafiltered YE
• Such extracts may be prepared by methods generally understood by those skilled in the art of bacteriological or animal cell culture medium formulation, or may be obtained commercially, for example from Sigma (Saint Louis, Missouri), Difco (Norwood, Massachusetts) or Quest International (Norwich, New York).
• YE or YEU are added to the basal or complete media described above at concentrations of about 10-8000 mg/liter, preferably about 10-100 mg/liter, and most preferably about 50-100 mg/liter.
• YE or YEU may be added to the basal media at these concentrations, in the absence of wheat-derived plant peptides, enzymatic digests of animal proteins and peptones, to formulate a suitable animal cell culture medium according to the present invention.
• the medium ingredients can be dissolved in a liquid carrier or maintained in dry form. If dissolved in a liquid carrier at the preferred concentrations shown in Table 1 (i.e., a "1X formulation"), the pH of the medium should be adjusted to about 7.0-7.5, preferably about 7.1-7.4, and most preferably about 7.1-7.3. The osmolarity of the medium should also be adjusted to about 275-350 mOsm, preferably about 285-325 mOsm, and most preferably about 300-325 mOsm. The type of liquid carrier and the method used to dissolve the ingredients into solution vary and can be determined by one of ordinary skill in the art with no more than routine experimentation. Typically, the medium ingredients can be added in any order.
• the solutions comprising ingredients are more concentrated than the concentration of the same ingredients in a 1X media formulation.
• the ingredients can be 10-fold more concentrated (10X formulation), 20-fold more concentrated (20X formulation), 25-fold more concentrated (25X formulation), 50-fold more concentrated (50X concentration), or 100-fold more concentrated (100X formulation). More highly concentrated formulations can be made, provided that the ingredients remain soluble and stable. See U.S. Patent No. 5,474,931 , which is directed to methods of solubilizing culture media components at high concentrations.
• the media ingredients are prepared as separate concentrated solutions, an appropriate (sufficient) amount of each concentrate is combined with a diluent to produce a 1X medium formulation.
• a diluent typically, the diluent used is water but other solutions including aqueous buffers, aqueous saline solution, or other aqueous solutions may be used according to the invention.
• the culture media of the present invention are typically sterilized to prevent unwanted contamination. Sterilization may be accomplished, for example, by filtration through a low protein-binding membrane filter of about 0.1-1.0 ⁇ m pore size (available commercially, for example, from Millipore, Bedford, Massachusetts) after admixing the concentrated ingredients to produce a sterile culture medium. Alternatively, concentrated subgroups of ingredients may be filter-sterilized and stored as sterile solutions. These sterile concentrates can then be mixed under aseptic conditions with a sterile diluent to produce a concentrated 1X sterile medium formulation. Autoclaving or other elevated temperature-based methods of sterilization are not favored, since many of the components of the present culture media are heat labile and will be irreversibly degraded by temperatures such as those achieved during most heat sterilization methods.
• the optimal concentration ranges for the basal medium ingredients are listed in Table 1. These ingredients can be combined to form the basal animal cell culture medium which is then supplemented with cytokines, plant peptides and optionally (but preferably) with YE, YEU and/or one or more plant lipids/fatty acids (or combinations thereof), to formulate the complete media of the present invention.
• concentration of a given ingredient can be increased or decreased beyond the range disclosed and the effect of the increased or decreased concentration can be determined using only routine experimentation.
• the concentrations of the ingredients of the medium of the present invention are the concentrations listed in the far right column of Table 1, supplemented with cytokines, plant peptides and YE, YEU and/or one or more plant lipids/fatty acids as described above.
• each of the components of the culture medium may react with one or more other components in the solution.
• the present invention encompasses the formulations disclosed in Table 1, supplemented as described above, as well as any reaction mixture which forms after these ingredients are combined.
• the optimization of the present media formulations was carried out using approaches described by Ham ( Ham, R.G., Methods for Preparation of Media, Supplements and Substrata for Serum-Free Animal Culture, Alan R. Liss, Inc., New York, pp. 3-21 (1984 )) and Waymouth ( Waymouth, C., Methods for Preparation of Media, Supplements and Substrata for Serum-Free Animal Culture, Alan R. Liss, Inc., New York, pp. 23-68 (1984 )).
• the optimal final concentrations for medium ingredients are typically identified either by empirical studies, in single component titration studies, or by interpretation of historical and current scientific literature. In single component titration studies, using animal cells, the concentration of a single medium component is varied while all other constituents and variables are kept constant and the effect of the single component on viability, growth or continued health of the animal cells is measured.
• the present invention also relates to methods for replacing or substituting animal-derived products with plant peptides, plant lipids, plant fatty acids, and/or enzymatic digests or extracts of yeast cells (or combinations thereof).
• plant- and/or yeast-derived nutrients may be substituted for any number of animal-derived culture medium components or substituents, including but not limited to blood-derived products, tissue/organ/gland extracts, animal-derived fatty acids and lipids, sterols, and lipoproteins.
• blood-derived products and tissue/organ extracts are substituted in the culture media of the invention using one or more of the above-described plant-derived peptides, while animal-derived fatty acids/lipids, sterols and lipoproteins are preferably substituted with one or more of the above-described plant-derived lipids/fatty acids.
• Typical blood-derived products that may be replaced in accordance with this aspect of the invention include but are not limited to serum (e.g., fetal bovine serum and calf serum, human serum, etc.), plasma, albumin (e.g., bovine serum albumin or human serum albumin), antibodies, fibrinogen, factor VIII, etc.
• Typical tissue/organ/gland extracts that may be replaced in accordance with this aspect of the invention include but are not limited to bovine pituitary extract (BPE), bovine brain extract, chicken embryo extract and bovine embryo extract.
• BPE bovine pituitary extract
• bovine brain extract bovine brain extract
• chicken embryo extract bovine embryo extract
• bovine embryo extract any animal-derived fatty acid or lipid, including saturated and unsaturated fatty acids/lipids that are well-known in the art, may be replaced with one or more of the above-described plant-derived lipids/fatty acids.
• animal-derived sterols e.g., cholesterol
• lipoproteins e.g., high- and low-density lipoproteins (HDLs and LDLs, respectively)
• HDLs and LDLs high- and low-density lipoproteins
• Other animal-derived medium components which may be replaced by one or more plant-derived nutrients in accordance with the invention can be easily determined by one of ordinary skill in the art by substituting one or more plant lipids/fatty acids, plant peptides and/or extracts/digests of yeast (or combinations thereof) and testing the effect of such substitution on cell growth by methods that will be familiar to the ordinarily skilled artisan (such as those methods described in the Examples below).
• Cells which can be cultivated in the medium of the present invention are those of animal origin, including but not limited to cells obtained from mammals, birds (avian), insects or fish.
• Mammalian cells particularly suitable for cultivation in the present media include those of human origin, which may be primary cells derived from a tissue sample, diploid cell strains, transformed cells or established cell lines (e.g., HeLa), each of which may optionally be diseased or genetically altered.
• mammalian cells such as hybridomas, CHO cells, COS cells, VERO cells, HeLa cells, 293 cells, PER-C6 cells, K562 cells, MOLT-4 cells, M1 cells, NS-1 cells, COS-7 cells, MDBK cells, MDCK cells, MRC-5 cells, WI-38 cells, WEHI cells, SP2/0 cells, BHK cells (including BHK-21 cells) and derivatives thereof, are also suitable for cultivation in the present media.
• stem cells and cells used in in vitro virus production may be cultivated in the media of the present invention.
• Insect cells particularly suitable for cultivation in the present media include those derived from Spodoptera species (e.g., Sf9 or Sf21, derived from Spodopterafrugiperda ) or Trichoplusa species (e.g., HIGH FIVE TM or MG1, derived from Trichoplusa ni). Tissues, organs, organ systems and organisms derived from animals or constructed in vitro or in vivo using methods routine in the art may similarly be cultivated in the culture media of the present invention.
• Spodoptera species e.g., Sf9 or Sf21, derived from Spodopterafrugiperda
• Trichoplusa species e.g., HIGH FIVE TM or MG1, derived from Trichoplusa ni.
• Tissues, organs, organ systems and organisms derived from animals or constructed in vitro or in vivo using methods routine in the art may similarly be cultivated in the culture media of the present invention.
• Animal cells for culturing by the present invention may be obtained commercially, for example from ATCC (Rockville, Maryland), Cell Systems, Inc. (Kirkland, Washington) or Invitrogen Corporation (San Diego, California). Alternatively, cells may be isolated directly from samples of animal tissue obtained via biopsy, autopsy, donation or other surgical or medical procedure.
• Tissue should be handled using standard sterile technique and a laminar flow safety cabinet. In the use and processing of all human tissue, the recommendations of the U.S. Department of Health and Human Services/Centers for Disease Control and Prevention should be followed ( Biosafety in Microbiological and Biomedical Laboratories, Richmond, J. Y. et al., Eds., U.S. Government Printing Office, Washington, D.C. 3rd Edition (1993 )). The tissue should be cut into small pieces (e.g., 0.5 x 0.5 cm) using sterile surgical instruments.
• the small pieces should be washed twice with sterile saline solution supplemented with antibiotics as above, and then may be optionally treated with an enzymatic solution (e.g., collagenase or trypsin solutions, each available commercially, for example, from Life Technologies, Inc., Rockville, Maryland) to promote dissociation of cells from the tissue matrix.
• an enzymatic solution e.g., collagenase or trypsin solutions, each available commercially, for example, from Life Technologies, Inc., Rockville, Maryland
• the mixture of dissociated cells and matrix molecules are washed twice with a suitable physiological saline or tissue culture medium (e.g., Dulbecco's Phosphate Buffered Saline without calcium and magnesium). Between washes, the cells are centrifuged ( e.g., at 200 x g ) and then resuspended in serum-free tissue culture medium. Aliquots are counted using an electronic cell counter (such as a Coulter Counter). Alternatively, the cells can be counted manually using a hemocytometer.
• tissue culture medium e.g., Dulbecco's Phosphate Buffered Saline without calcium and magnesium.
• the isolated cells can be plated according to the experimental conditions determined by the investigator.
• the examples below demonstrate at least one functional set of culture conditions useful for cultivation of certain mammalian cells. It is to be understood, however, that the optimal plating and culture conditions for a given animal cell type can be determined by one of ordinary skill in the art using only routine experimentation.
• cells can be plated onto the surface of culture vessels without attachment factors.
• the vessels can be precoated with natural, recombinant or synthetic attachment factors or peptide fragments (e.g., collagen or fibronectin, or natural or synthetic fragments thereof).
• Isolated cells can also be seeded into or onto a natural or synthetic three-dimensional support matrix such as a preformed collagen gel or a synthetic biopolymeric material, or onto feeder layers of cells.
• a natural or synthetic three-dimensional support matrix such as a preformed collagen gel or a synthetic biopolymeric material, or onto feeder layers of cells.
• Use of attachment factors or a support matrix with the medium of the present invention will enhance cultivation of many attachment-dependent cells in the absence of serum supplementation.
• the cell seeding densities for each experimental condition can be optimized for the specific culture conditions being used. For routine culture in plastic culture vessels, an initial seeding density of 0.1-1.0 X 10 5 cells per cm 2 or about 1.5X the plating concentration routinely used for the same cells in serum supplemented media is preferable.
• Mammalian cells are typically cultivated in a cell incubator at about 37°C, while the optimal temperatures for cultivation of avian, nematode and insect cells are typically somewhat lower and are well-known to those of ordinary skill in the art.
• the incubator atmosphere should be humidified for cultivation of animal cells, and should contain about 3-10% carbon dioxide in air.
• Culture medium pH should be in the range of about 7.1-7.6, preferably about 7.1-7.4, and most preferably about 7.1-7.3.
• Cells in closed or batch culture should undergo complete medium exchange (i.e., replacing spent media with fresh media) about every 2-3 days, or more or less frequently as required by the specific cell type.
• Cells in perfusion culture e.g., in bioreactors or fermenters
• the cell culture media of the present invention may also be used to produce cell culture compositions comprising the present media and an animal cell.
• Animal cells preferably used in such compositions include, but are not limited to, cells obtained from mammals, birds (avian), insects or fish.
• Mammalian cells particularly suitable for use in such compositions include those of human origin, which may be primary cells derived from a tissue sample, diploid cell strains, transformed cells or established cell lines (e.g., HeLa), each of which may optionally be diseased or genetically altered.
• mammalian cells such as hybridomas, CHO cells, COS cells, VERO cells, HeLa cells, 293 cells, PER-C6 cells, K562 cells, MOLT-4 cells, M1 cells, NS-1 cells, COS-7 cells, MDBK cells, MDCK cells, MRC-5 cells, WI-38 cells, SP2/0 cells, BHK cells (including BHK-21 cells) and derivatives thereof, are also suitable for use in forming the cell culture compositions of the present invention.
• mammalian cells such as hybridomas, CHO cells, COS cells, VERO cells, HeLa cells, 293 cells, PER-C6 cells, K562 cells, MOLT-4 cells, M1 cells, NS-1 cells, COS-7 cells, MDBK cells, MDCK cells, MRC-5 cells, WI-38 cells, SP2/0 cells, BHK cells (including BHK-21 cells) and derivatives thereof, are also suitable for use in forming the cell culture compositions of the present invention.
• Insect cells particularly suitable for use in forming such compositions include those derived from Spodoptera species (e.g., Sf9 or Sf21, derived from Spodoptera frugiperda) or Trichoplusa species (e.g., HIGH FIVE TM or MG1, derived from Trichoplusa ni ). Tissues, organs, organ systems and organisms derived from animals or constructed in vitro or in vivo using methods routine in the art may similarly be used to form the cell culture compositions of the present invention. These cell culture compositions may be used in a variety of medical (including diagnostic and therapeutic), industrial, forensic and research applications requiring ready-to-use cultures of animal cells in serum-free media.
• Spodoptera species e.g., Sf9 or Sf21, derived from Spodoptera frugiperda
• Trichoplusa species e.g., HIGH FIVE TM or MG1, derived from Trichoplusa ni .
• VERO cultures (ATCC) were plated in 25 cm 2 cell culture flasks in duplicate in each medium at about 2.5 x 10 5 cells per flask in 5 ml of medium. No attachment factors or coating of the plastic surface are required for the culture of VERO cells. At 3 to 4 days the cells were removed using standard cell culture techniques. The surface of the culture was first washed with Dulbecco's Phosphate Buffered Saline (DPBS) and then 1.0 ml Trypsin-EDTA (Life Technologies, Inc.; Rockville, Maryland) was added. The digest was allowed to sit on the cell surface for 3 to 5 minutes or until the cells rounded up and began to detach from the surface of the flask.
• DPBS Dulbecco's Phosphate Buffered Saline
• Trypsin-EDTA Life Technologies, Inc.; Rockville, Maryland
• the cells were completely detached by vigorous agitation against the palm of the hand and then 1.5 ml of soybean trypsin inhibitor was added to quickly neutralize enzymatic activity.
• the cells were counted under the microscope using trypan blue straining solution and new cultures plated at 2.5 x 10 5 cells per 25 cm 2 flask. Incubation was at 37°C in 5% CO 2 in air. The cultures were passaged for a total of 4 subcultures and the mean cells per subculture determined from the counts of the final 3 subcultures (P2 + P3 + P4 ⁇ 3).
• ddH 2 O distilled, deionized water
• trace elements from 1000x stock
• L-alanine (0.22 g)
• L-arginine ⁇ HCl 9.75 g
• L-asparagine ⁇ HCl (1.02 g)
• L-aspartic acid 0.332 g
• L-cysteine ⁇ HCl ⁇ H 2 O 0.10 g
• L-cystine ⁇ HCl 0.87 g
• glycine (0.188 g)
• L-glutamic acid 0.268 g
• L-histidine ⁇ HCl ⁇ H 2 O 1.707 g
• L-isoleucine 4284 g
• L-leucine 4.511 g
• L-lysine ⁇ HCl 5.640 g
• L-methionine 1.266 g
• L-phenyl 5N HCl
• ATP 0.025 g
• uracil 0.0075 g
• PABA 0.0012 g
• D-Ca ++ -pantothenate 0.05 g
• riboflavin 0.005 g
• NaCl 142.50 g
• CaCl 2 3.00 g
• MgCl 2 3.125 g
• EGF 0.00025 g
• the solution was again gently mixed for about 15 minutes, during which time a 20 ml volume of absolute ethanol was obtained, to which were added vitamin A acetate (0.0035 g), vitamin D2 (0.0025 g), menadione (0.00025 g), lipoic acid (0.0019 g) and linoleic acid (0.00088 g).
• the ethanol solution was added to the 20 liter medium solution from above, and the medium solution was gently mixed for about 5 minutes.
• biotin 0.0019 g
• folic acid 0.05 g
• hypoxanthine ⁇ Na 0.0415 g
• xanthine ⁇ Na 0.0075 g
• insulin-Zn ++ 0.125 g
• the pH of the solution was then adjusted with 5N HC1 or 5N NaOH to about 7.15 ⁇ 0.50.
• adenine sulfate (0.25 g), D-glucose (97.56 g), choline chloride (0.20 g), i -inositol (0.45 g), nicotinic acid (0.00062 g), niacinamide (0.05 g), sodium pyruvate (3.75 g), 2-deoxyribose (0.0125 g), KCl (8.0 g), putrescine•2HCl (0.0015 g), phosphoethanolamine (0.03 g), vitamin B12 (0.0125 g), HEPES (45.0 g), NaHCO 3 (55.0 g) and phenol red (0.10g).
• This solution was gently mixed for about 10-15 minutes, the pH was then adjusted with 5N HCl or 5N NaOH to about 7.20 ⁇ 0.10, and ddH 2 O was added to bring the final volume of the solution up to 25.0 liters.
• the osmolarity of the solution was determined to be about 310 ⁇ 10 mOsm.
• This basal medium formulation was then filtered through a low protein-binding filter cartridge and stored at 4°C in conditions of diminished light until use.
• VERO cells were cultured in the various medium formulations, and cell counts determined, as described above in Materials and Methods, and were compared to those obtained in basal medium that was unsupplemented (negative control) or supplemented with 500 mg/liter human serum albumin (HSA; positive control). Results shown in Table 2 demonstrate mean cell count per 25 cm 2 flask over 3 subcultures and relative growth efficiency (RGE) for each of the medium formulations; RGE was calculated by dividing the mean cell count for a given medium formulation by that for the HSA control. Table 2. Non-Animal Peptide Screen. Supplement Mean Cell Count, x 10 5 RGE HSA 44.9 100 Yeast Extract 31.1 69 Wheat Hydrolysate 1 12.4 28 Wheat Hydrolysate 2 12.4 28 Soy Hydrolysate 31.3 70 Rice Hydrolysate 35.9 80
• Example 1 To examine the effect of growth factor concentration on the performance of the culture media, recombinant human EGF was added to the basal media of Example 1 at various concentrations. These media were then used to examine VERO cell growth as described above. Cell counts were compared to those obtained in basal medium that was unsupplemented (negative control) or to EMEM supplemented with 5% FBS (positive control). Results shown in Table 6 demonstrate mean cell count and relative growth efficiency (RGE) for each of the EGF concentrations; RGE was calculated as described in Example 2. Table 6. Titration of EGF.
• EGF Mean Cell Count, x 10 5 RGE* 0 5.1 100 5 7.0 137 6 6.0 118 7 7.1 139 8 7.3 143 9 7.4 145 10 6.8 133 * as % of 0 mg/L control.
• an optimal culture medium formulation for supporting the cultivation of animal cells is the basal medium formulation shown in Table 1, supplemented with EGF at 5-10 mg/liter, yeast extract (preferably yeast extract ultrafiltrate) at 50-100 mg/liter, and at least one plant peptide (preferably rice peptides or hydrolysate) at 100-200 mg/liter.
• Table 9 shows the use of the medium to grow BHK-21 cells in suspension on a shaker platform.
• 0.2% PLURONIC F68 was added to both the test medium and the EMEM FBS 5% control to reduce shear damage. Counts were made at 72, 96 and 120 hours. As can be seen in Table 9 the test medium performed as well as or better than the control. By 120 hrs the viability began dropping much more rapidly in the control serum-supplemented medium as compared to this preferred embodiment of the present invention.
• Table 9 Growth of BHK-21 Cells in Suspension in Shaker Flasks. Time (hrs) Viable cells/ml x 10 5 EMEM 5% FBS control Preferred Embodiment of Present Invention 0 3.2 3.2 72 7.1 7.8 96 9.0 10.4 120 3.7 8.0
• culture media made as described in Example 1 were used to culture VERO cells.
• Cells were plated in T-25 flasks into culture media that were not supplemented with plant-derived lipids or fatty acids (control) or that were supplemented with 5 ⁇ g/ml, 0.5 ⁇ g/ml or 0.05 ⁇ g/ml of one of the following plant lipid or fatty acid mixes obtained from Matreya, Inc. (Pleasant Gap, Pennsylvania), having constituents present in the indicated percentages:

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